Ten Ways to Increase the Sensitivity of Northern Hybridizations

Increase the Amount of RNA Loaded in Each Lane
Use Poly(A) RNA Instead of Total RNA
Switch From a Traditional Hybridization Buffer to ULTRAhyb
If Using a Traditional Hybridization Buffer, Switch From DNA to RNA Probes
Use Downward Alkaline Capillary Transfer Instead of Neutral Capillary Transfer
Use an Optimal Hybridization Temperature
Use Freshly Synthesized Radiolabeled Probes
Use High Specific Activity Probes
Increase Exposure Time
Follow the Manufacturer’s Recommendations to Crosslink the RNA to the Membrane

Increase the Amount of RNA Loaded in Each Lane

Up to 30 µg of total RNA can be loaded in each lane.

Use Poly(A) RNA Instead of Total RNA

For very rare messages you may need to use poly(A) RNA instead of total RNA. 10 µg of mRNA is equivalent to 300–350 µg of total RNA. (mRNA comprises only about 0.5–3% of total RNA.)

Switch From a Traditional Hybridization Buffer to ULTRAhyb

ULTRAhyb Ultrasensitive Hybridization Buffer can increase the sensitivity of a blot hybridization up to 100-fold.

If Using a Traditional Hybridization Buffer, Switch From DNA to RNA Probes

RNA probes are more sensitive than DNA probes when using traditional hybridization buffer. ULTRAhyb Ultrasensitive Hybridization Buffer, however, substantially increases the sensitivity of DNA probes making them as sensitive as RNA probes.

Use Downward Alkaline Capillary Transfer Instead of Neutral Capillary Transfer

Alkaline transfer nicks the RNA, increasing sensitivity by more efficiently moving RNA, especially larger transcripts, from the gel to the membrane. Downward transfer does not crush the gel and makes use of gravity to speed up the process. (Ambion’s NorthernMax Kits include reagents for alkaline transfer.)

Use an Optimal Hybridization Temperature

Temperatures of 42°C for DNA probes and 68°C for RNA probes usually give excellent results in 50% formamide-based hybridization buffers. Hybridization conditions for probes that have an unusually high GC or AT content or probes with a high degree of mismatch with the target should be determined empirically.

Use Freshly Synthesized Radiolabeled Probes

High specific activity probes degrade rapidly due to autoradiolysis, resulting in low signal and/or high background.

Use High Specific Activity Probes

The specific activity of the probe should be at least 10⁸ cpm/µg and preferably > 10⁹ cpm/µg.

Increase Exposure Time

Low copy number RNAs can take more than 3 days to show up using ³²P-labeled probes at –70°C with intensifying screens.

Follow the Manufacturer’s Recommendations to Crosslink the RNA to the Membrane

It is possible to over or under crosslink the RNA by not using the proper procedure.

Learn more about Northern Blotting

For Research Use Only. Not for use in diagnostic procedures.

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